pRARE-MBP-DEST
(Plasmid #84650)

• Purpose: (Empty Backbone) Gateway cloning vector expresses MBP-tagged proteins under the control of the IPTG– inducible ptac promoter and also expresses several tRNAs that are rare in E. coli.
• Depositing Lab: Neil Olszewski
• Publication: Steiner et al Plant Cell. 2012 Jan;24(1):96-108. doi: 10.1105/tpc.111.093518. Epub 2012 Jan 20.

Backbone

• Vector backbone: pRARE
• Backbone manufacturer: EMD Chemicals
• Modifications to backbone: malE expression cassette of pMAL-c2 (New England Biolabs) was modified for Gateway cloning. The region containing the lacIq gene and modified malE expression cassette was then subcloned into the pRARE plasmid.
• Vector type: Bacterial Expression
• Promoter: tac
• Tag / Fusion Protein:
  • MBP (N terminal on backbone)

Growth in Bacteria

• Bacterial Resistance(s): Chloramphenicol and Kanamycin, 25 & 50 μg/mL
• Growth Temperature: 37°C
• Growth Strain(s): DB3.1
• Copy number: Unknown

Cloning Information

• Cloning method: Gateway Cloning
• 5′ sequencing primer: MBP-F
• 3′ sequencing primer: pBAD-R

Resource Information

• Supplemental Documents:
  • annotated sequence

Terms and Licenses

• Academic/Nonprofit Terms:
  • UBMTA
• Industry Terms:
  • Not Available to Industry

How to cite this plasmid

• For your Materials & Methods section:

  pRARE-MBP-DEST was a gift from Neil Olszewski (Addgene plasmid # 84650 ; http://n2t.net/addgene:84650 ; RRID:Addgene_84650)

• For your References section:

  The Arabidopsis O-linked N-acetylglucosamine transferase SPINDLY interacts with class I TCPs to facilitate cytokinin responses in leaves and flowers. Steiner E, Efroni I, Gopalraj M, Saathoff K, Tseng TS, Kieffer M, Eshed Y, Olszewski N, Weiss D. Plant Cell. 2012 Jan;24(1):96-108. doi: 10.1105/tpc.111.093518. Epub 2012 Jan 20. 10.1105/tpc.111.093518 PubMed 22267487